xfect clontech reagents Search Results


clontech xfect transfection  (TaKaRa)
97
TaKaRa clontech xfect transfection
Clontech Xfect Transfection, supplied by TaKaRa, used in various techniques. Bioz Stars score: 97/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/clontech xfect transfection/product/TaKaRa
Average 97 stars, based on 1 article reviews
clontech xfect transfection - by Bioz Stars, 2026-03
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xfect mesc transfection reagent  (TaKaRa)
94
TaKaRa xfect mesc transfection reagent
dCas9VP160 activates endogenous genes. (A) Protein architecture of dCas9VP160 compared to VP48. (B) Schematic of the human IL1RN promoter region. Locations of transcription start site (TSS) and start codon (ATG) are indicated. Short lines with number indicate targeting sites of the sgRNAs. (C) Activation of human IL1RN expression in HEK293T cells. Cells were analyzed by qRT-PCR 2 days after <t>transfection</t> with dCas9VP160 and the indicated sgRNAs. (D) Schematic of the human SOX2 promoter region. Locations of TSS and start codon (ATG) are indicated. Short lines with number indicate targeting sites of sgRNAs. (E) Activation of SOX2 . Cells were analyzed by qRT-PCR 2 days after transfection with dCas9VP160 and the indicated sgRNAs. (F) Schematic of the human OCT4 promoter region. Locations of transcription start site (TSS) and start codon (ATG) are indicated. Short lines with number indicate targeting sites of sgRNAs. (G) Activation of OCT4 . Cells transfected with dCas9VP160 and the indicated sgRNAs were analyzed by qRT-PCR 2 days later. sgTetO-mut, negative control sgRNA. Error bars show SD among triplicates.
Xfect Mesc Transfection Reagent, supplied by TaKaRa, used in various techniques. Bioz Stars score: 94/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/xfect mesc transfection reagent/product/TaKaRa
Average 94 stars, based on 1 article reviews
xfect mesc transfection reagent - by Bioz Stars, 2026-03
94/100 stars
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xfect protein transfection reagent  (TaKaRa)
93
TaKaRa xfect protein transfection reagent
dCas9VP160 activates endogenous genes. (A) Protein architecture of dCas9VP160 compared to VP48. (B) Schematic of the human IL1RN promoter region. Locations of transcription start site (TSS) and start codon (ATG) are indicated. Short lines with number indicate targeting sites of the sgRNAs. (C) Activation of human IL1RN expression in HEK293T cells. Cells were analyzed by qRT-PCR 2 days after <t>transfection</t> with dCas9VP160 and the indicated sgRNAs. (D) Schematic of the human SOX2 promoter region. Locations of TSS and start codon (ATG) are indicated. Short lines with number indicate targeting sites of sgRNAs. (E) Activation of SOX2 . Cells were analyzed by qRT-PCR 2 days after transfection with dCas9VP160 and the indicated sgRNAs. (F) Schematic of the human OCT4 promoter region. Locations of transcription start site (TSS) and start codon (ATG) are indicated. Short lines with number indicate targeting sites of sgRNAs. (G) Activation of OCT4 . Cells transfected with dCas9VP160 and the indicated sgRNAs were analyzed by qRT-PCR 2 days later. sgTetO-mut, negative control sgRNA. Error bars show SD among triplicates.
Xfect Protein Transfection Reagent, supplied by TaKaRa, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/xfect protein transfection reagent/product/TaKaRa
Average 93 stars, based on 1 article reviews
xfect protein transfection reagent - by Bioz Stars, 2026-03
93/100 stars
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xfect rna transfection reagent  (TaKaRa)
95
TaKaRa xfect rna transfection reagent
dCas9VP160 activates endogenous genes. (A) Protein architecture of dCas9VP160 compared to VP48. (B) Schematic of the human IL1RN promoter region. Locations of transcription start site (TSS) and start codon (ATG) are indicated. Short lines with number indicate targeting sites of the sgRNAs. (C) Activation of human IL1RN expression in HEK293T cells. Cells were analyzed by qRT-PCR 2 days after <t>transfection</t> with dCas9VP160 and the indicated sgRNAs. (D) Schematic of the human SOX2 promoter region. Locations of TSS and start codon (ATG) are indicated. Short lines with number indicate targeting sites of sgRNAs. (E) Activation of SOX2 . Cells were analyzed by qRT-PCR 2 days after transfection with dCas9VP160 and the indicated sgRNAs. (F) Schematic of the human OCT4 promoter region. Locations of transcription start site (TSS) and start codon (ATG) are indicated. Short lines with number indicate targeting sites of sgRNAs. (G) Activation of OCT4 . Cells transfected with dCas9VP160 and the indicated sgRNAs were analyzed by qRT-PCR 2 days later. sgTetO-mut, negative control sgRNA. Error bars show SD among triplicates.
Xfect Rna Transfection Reagent, supplied by TaKaRa, used in various techniques. Bioz Stars score: 95/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/xfect rna transfection reagent/product/TaKaRa
Average 95 stars, based on 1 article reviews
xfect rna transfection reagent - by Bioz Stars, 2026-03
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xfect transfection reagents  (Sartorius AG)
86
Sartorius AG xfect transfection reagents
The CNS and reference gene (RG) promoters are selectively activated by specific single guide RNAs (sgRNAs) designed to target them. ( a ) Schematic representation of the PPARGC1A locus showing the CNS and RG promoters (top), locations of sgRNAs used for transfections; CNS-specific exons B1 , B4 and B5 in color; the structure of the RG is displayed on the right; CNS-specific transcripts and RG transcripts are shown below; * pink or red lines refer to alternatively spliced transcripts encoding stop codons in exon 7A or in an extension of exon 3, respectively. ( b , c ) Selective effects of individual sgRNAs targeting the RG or CNS promoters on transcription initiation; individual sgRNAs or their mixtures were transfected into clonal SH-SY5Y cells expressing CRISPR-associated deactivated (dCas9) protein fused to the tripartite transcriptional activator VPR and levels of E1E2 and B1B4 transcripts selective for RG or CNS promoter activation were measured by qRT-PCR 36 h after <t>transfection.</t> Log-fold levels are expressed relative to transcript levels of the clonal cells transfected with scrambled sgRNA. Interactions of all sgRNA mixtures shown were significant ( p < 0.001) when the use of three, two, or one sgRNA was compared. ( d ) Effects of sgRNA transfections on CNS-specific and RG transcript levels and levels of transcripts encoding truncated isoforms and initiated at either promoter.
Xfect Transfection Reagents, supplied by Sartorius AG, used in various techniques. Bioz Stars score: 86/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/xfect transfection reagents/product/Sartorius AG
Average 86 stars, based on 1 article reviews
xfect transfection reagents - by Bioz Stars, 2026-03
86/100 stars
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xfect tm transfection reagent  (Becton Dickinson)
90
Becton Dickinson xfect tm transfection reagent
The CNS and reference gene (RG) promoters are selectively activated by specific single guide RNAs (sgRNAs) designed to target them. ( a ) Schematic representation of the PPARGC1A locus showing the CNS and RG promoters (top), locations of sgRNAs used for transfections; CNS-specific exons B1 , B4 and B5 in color; the structure of the RG is displayed on the right; CNS-specific transcripts and RG transcripts are shown below; * pink or red lines refer to alternatively spliced transcripts encoding stop codons in exon 7A or in an extension of exon 3, respectively. ( b , c ) Selective effects of individual sgRNAs targeting the RG or CNS promoters on transcription initiation; individual sgRNAs or their mixtures were transfected into clonal SH-SY5Y cells expressing CRISPR-associated deactivated (dCas9) protein fused to the tripartite transcriptional activator VPR and levels of E1E2 and B1B4 transcripts selective for RG or CNS promoter activation were measured by qRT-PCR 36 h after <t>transfection.</t> Log-fold levels are expressed relative to transcript levels of the clonal cells transfected with scrambled sgRNA. Interactions of all sgRNA mixtures shown were significant ( p < 0.001) when the use of three, two, or one sgRNA was compared. ( d ) Effects of sgRNA transfections on CNS-specific and RG transcript levels and levels of transcripts encoding truncated isoforms and initiated at either promoter.
Xfect Tm Transfection Reagent, supplied by Becton Dickinson, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/xfect tm transfection reagent/product/Becton Dickinson
Average 90 stars, based on 1 article reviews
xfect tm transfection reagent - by Bioz Stars, 2026-03
90/100 stars
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Image Search Results


dCas9VP160 activates endogenous genes. (A) Protein architecture of dCas9VP160 compared to VP48. (B) Schematic of the human IL1RN promoter region. Locations of transcription start site (TSS) and start codon (ATG) are indicated. Short lines with number indicate targeting sites of the sgRNAs. (C) Activation of human IL1RN expression in HEK293T cells. Cells were analyzed by qRT-PCR 2 days after transfection with dCas9VP160 and the indicated sgRNAs. (D) Schematic of the human SOX2 promoter region. Locations of TSS and start codon (ATG) are indicated. Short lines with number indicate targeting sites of sgRNAs. (E) Activation of SOX2 . Cells were analyzed by qRT-PCR 2 days after transfection with dCas9VP160 and the indicated sgRNAs. (F) Schematic of the human OCT4 promoter region. Locations of transcription start site (TSS) and start codon (ATG) are indicated. Short lines with number indicate targeting sites of sgRNAs. (G) Activation of OCT4 . Cells transfected with dCas9VP160 and the indicated sgRNAs were analyzed by qRT-PCR 2 days later. sgTetO-mut, negative control sgRNA. Error bars show SD among triplicates.

Journal: Cell Research

Article Title: Multiplexed activation of endogenous genes by CRISPR-on, an RNA-guided transcriptional activator system

doi: 10.1038/cr.2013.122

Figure Lengend Snippet: dCas9VP160 activates endogenous genes. (A) Protein architecture of dCas9VP160 compared to VP48. (B) Schematic of the human IL1RN promoter region. Locations of transcription start site (TSS) and start codon (ATG) are indicated. Short lines with number indicate targeting sites of the sgRNAs. (C) Activation of human IL1RN expression in HEK293T cells. Cells were analyzed by qRT-PCR 2 days after transfection with dCas9VP160 and the indicated sgRNAs. (D) Schematic of the human SOX2 promoter region. Locations of TSS and start codon (ATG) are indicated. Short lines with number indicate targeting sites of sgRNAs. (E) Activation of SOX2 . Cells were analyzed by qRT-PCR 2 days after transfection with dCas9VP160 and the indicated sgRNAs. (F) Schematic of the human OCT4 promoter region. Locations of transcription start site (TSS) and start codon (ATG) are indicated. Short lines with number indicate targeting sites of sgRNAs. (G) Activation of OCT4 . Cells transfected with dCas9VP160 and the indicated sgRNAs were analyzed by qRT-PCR 2 days later. sgTetO-mut, negative control sgRNA. Error bars show SD among triplicates.

Article Snippet: mESCs from mice carrying a Dox-inducible Musashi-1 (MSI1) allele in the Col1A1 locus were transfected with dCas9VP48 using Xfect mESC transfection reagent (Clontech) or were cultured in mouse ES medium with 2 μg/ml Doxycycline.

Techniques: Activation Assay, Expressing, Quantitative RT-PCR, Transfection, Negative Control

Multiple exogenous and endogenous genes were simultaneously activated by CRISPR-on. (A) One exogenous and two endogenous genes were simultaneously activated by CRISPR-on. Cells were analyzed by qRT-PCR 2 days after transfection with dCas9VP160 and the indicated sgRNAs. (B) Three endogenous genes, SOX2 , IL1RN and OCT4 , can be simultaneously activated by dCas9VP160/sgRNAs. Cells were transfected with dCas9VP160 and the indicated sgRNAs and were analyzed by qRT-PCR 2 days after transfection. The Last three sets of bars represent triple activation experiments using sgSOX2, sgOCT4 and sgIL1RN with three different ratios of sgSOX2:sgIL1RN, keeping the amount of sgOCT4 constant, as indicated by numbers above line. sgTetO-mut, negative control sgRNA. Error bars show SD among triplicates.

Journal: Cell Research

Article Title: Multiplexed activation of endogenous genes by CRISPR-on, an RNA-guided transcriptional activator system

doi: 10.1038/cr.2013.122

Figure Lengend Snippet: Multiple exogenous and endogenous genes were simultaneously activated by CRISPR-on. (A) One exogenous and two endogenous genes were simultaneously activated by CRISPR-on. Cells were analyzed by qRT-PCR 2 days after transfection with dCas9VP160 and the indicated sgRNAs. (B) Three endogenous genes, SOX2 , IL1RN and OCT4 , can be simultaneously activated by dCas9VP160/sgRNAs. Cells were transfected with dCas9VP160 and the indicated sgRNAs and were analyzed by qRT-PCR 2 days after transfection. The Last three sets of bars represent triple activation experiments using sgSOX2, sgOCT4 and sgIL1RN with three different ratios of sgSOX2:sgIL1RN, keeping the amount of sgOCT4 constant, as indicated by numbers above line. sgTetO-mut, negative control sgRNA. Error bars show SD among triplicates.

Article Snippet: mESCs from mice carrying a Dox-inducible Musashi-1 (MSI1) allele in the Col1A1 locus were transfected with dCas9VP48 using Xfect mESC transfection reagent (Clontech) or were cultured in mouse ES medium with 2 μg/ml Doxycycline.

Techniques: CRISPR, Quantitative RT-PCR, Transfection, Activation Assay, Negative Control

The CNS and reference gene (RG) promoters are selectively activated by specific single guide RNAs (sgRNAs) designed to target them. ( a ) Schematic representation of the PPARGC1A locus showing the CNS and RG promoters (top), locations of sgRNAs used for transfections; CNS-specific exons B1 , B4 and B5 in color; the structure of the RG is displayed on the right; CNS-specific transcripts and RG transcripts are shown below; * pink or red lines refer to alternatively spliced transcripts encoding stop codons in exon 7A or in an extension of exon 3, respectively. ( b , c ) Selective effects of individual sgRNAs targeting the RG or CNS promoters on transcription initiation; individual sgRNAs or their mixtures were transfected into clonal SH-SY5Y cells expressing CRISPR-associated deactivated (dCas9) protein fused to the tripartite transcriptional activator VPR and levels of E1E2 and B1B4 transcripts selective for RG or CNS promoter activation were measured by qRT-PCR 36 h after transfection. Log-fold levels are expressed relative to transcript levels of the clonal cells transfected with scrambled sgRNA. Interactions of all sgRNA mixtures shown were significant ( p < 0.001) when the use of three, two, or one sgRNA was compared. ( d ) Effects of sgRNA transfections on CNS-specific and RG transcript levels and levels of transcripts encoding truncated isoforms and initiated at either promoter.

Journal: International Journal of Molecular Sciences

Article Title: Selective Activation of CNS and Reference PPARGC1A Promoters Is Associated with Distinct Gene Programs Relevant for Neurodegenerative Diseases

doi: 10.3390/ijms22073296

Figure Lengend Snippet: The CNS and reference gene (RG) promoters are selectively activated by specific single guide RNAs (sgRNAs) designed to target them. ( a ) Schematic representation of the PPARGC1A locus showing the CNS and RG promoters (top), locations of sgRNAs used for transfections; CNS-specific exons B1 , B4 and B5 in color; the structure of the RG is displayed on the right; CNS-specific transcripts and RG transcripts are shown below; * pink or red lines refer to alternatively spliced transcripts encoding stop codons in exon 7A or in an extension of exon 3, respectively. ( b , c ) Selective effects of individual sgRNAs targeting the RG or CNS promoters on transcription initiation; individual sgRNAs or their mixtures were transfected into clonal SH-SY5Y cells expressing CRISPR-associated deactivated (dCas9) protein fused to the tripartite transcriptional activator VPR and levels of E1E2 and B1B4 transcripts selective for RG or CNS promoter activation were measured by qRT-PCR 36 h after transfection. Log-fold levels are expressed relative to transcript levels of the clonal cells transfected with scrambled sgRNA. Interactions of all sgRNA mixtures shown were significant ( p < 0.001) when the use of three, two, or one sgRNA was compared. ( d ) Effects of sgRNA transfections on CNS-specific and RG transcript levels and levels of transcripts encoding truncated isoforms and initiated at either promoter.

Article Snippet: For the stable integration of dCas9-VPR into the genome of cell lines, pLenti-EF1a-dCas9-SAM plasmids (ABM) along with the trans-complementation plasmids pMD2.G expressing VSV-G envelope and phCMV-8.91 expressing GAG/POL were transfected into HEK293T cells using jetPEI or Xfect transfection reagents (Polyplus Transfection T or Clontech, Mountain View, CA, USA) in serum and antibiotic free medium.

Techniques: Transfection, Expressing, CRISPR, Activation Assay, Quantitative RT-PCR

RNA sequencing confirms the predicted structure of transcripts generated by activation of the RG or CNS promoters and reveals differentially expressed genes (DEGs) for either promoter activation. ( a ) Sashimi plots of PPARGC1A transcripts generated by transfection of clonal SH-SY5Y cells expressing dCas9-VPR with sgRNAs activating the RG or the CNS promoters or with scrambled sgRNAs, each merged from three biological replicates; read densities across exons are normalized to obtain comparable measures of expression above the x -axis and normalized single-end junction reads are shown as arcs below the x -axis; structure of visualized exons is shown at the bottom. ( b , c ) Volcano plots of DEGs in cells with RG or CNS activated promoters, respectively, in comparison to cells transfected with scrambled sgRNAs. The top 20 most DEGS are highlighted.

Journal: International Journal of Molecular Sciences

Article Title: Selective Activation of CNS and Reference PPARGC1A Promoters Is Associated with Distinct Gene Programs Relevant for Neurodegenerative Diseases

doi: 10.3390/ijms22073296

Figure Lengend Snippet: RNA sequencing confirms the predicted structure of transcripts generated by activation of the RG or CNS promoters and reveals differentially expressed genes (DEGs) for either promoter activation. ( a ) Sashimi plots of PPARGC1A transcripts generated by transfection of clonal SH-SY5Y cells expressing dCas9-VPR with sgRNAs activating the RG or the CNS promoters or with scrambled sgRNAs, each merged from three biological replicates; read densities across exons are normalized to obtain comparable measures of expression above the x -axis and normalized single-end junction reads are shown as arcs below the x -axis; structure of visualized exons is shown at the bottom. ( b , c ) Volcano plots of DEGs in cells with RG or CNS activated promoters, respectively, in comparison to cells transfected with scrambled sgRNAs. The top 20 most DEGS are highlighted.

Article Snippet: For the stable integration of dCas9-VPR into the genome of cell lines, pLenti-EF1a-dCas9-SAM plasmids (ABM) along with the trans-complementation plasmids pMD2.G expressing VSV-G envelope and phCMV-8.91 expressing GAG/POL were transfected into HEK293T cells using jetPEI or Xfect transfection reagents (Polyplus Transfection T or Clontech, Mountain View, CA, USA) in serum and antibiotic free medium.

Techniques: RNA Sequencing Assay, Generated, Activation Assay, Transfection, Expressing, Comparison

Differentially expressed genes resulting from activation of the RG or CNS promoters reveal promoter selectivity with partial overlap. ( a ) Venn diagram of differentially expressed genes (DEGS) produced by transfection of clonal SH-SY5Y cells expressing dCas9-VPR with sgRNAs activating the RG or the CNS promoters are compared with cells transfected with scrambled sgRNAs. ( b , c ) Top canonical signaling pathways for DEGs after RG or CNS promoter activation, respectively. ( d ) Top nervous system signaling pathways for DEGs after CNS promoter activation; red lines refer to adjusted p -values of 0.05; z -scores > 2.0 or <−2.0 are significant and indicate the direction for the expected entity; n.a, not available; B-H, Bernini-Hochberg adjusted p -values for multiple testing.

Journal: International Journal of Molecular Sciences

Article Title: Selective Activation of CNS and Reference PPARGC1A Promoters Is Associated with Distinct Gene Programs Relevant for Neurodegenerative Diseases

doi: 10.3390/ijms22073296

Figure Lengend Snippet: Differentially expressed genes resulting from activation of the RG or CNS promoters reveal promoter selectivity with partial overlap. ( a ) Venn diagram of differentially expressed genes (DEGS) produced by transfection of clonal SH-SY5Y cells expressing dCas9-VPR with sgRNAs activating the RG or the CNS promoters are compared with cells transfected with scrambled sgRNAs. ( b , c ) Top canonical signaling pathways for DEGs after RG or CNS promoter activation, respectively. ( d ) Top nervous system signaling pathways for DEGs after CNS promoter activation; red lines refer to adjusted p -values of 0.05; z -scores > 2.0 or <−2.0 are significant and indicate the direction for the expected entity; n.a, not available; B-H, Bernini-Hochberg adjusted p -values for multiple testing.

Article Snippet: For the stable integration of dCas9-VPR into the genome of cell lines, pLenti-EF1a-dCas9-SAM plasmids (ABM) along with the trans-complementation plasmids pMD2.G expressing VSV-G envelope and phCMV-8.91 expressing GAG/POL were transfected into HEK293T cells using jetPEI or Xfect transfection reagents (Polyplus Transfection T or Clontech, Mountain View, CA, USA) in serum and antibiotic free medium.

Techniques: Activation Assay, Produced, Transfection, Expressing

CNS-specific and reference PGC-1α proteins affect exon usage via distinct and similar mechanisms. ( a ) Venn diagram showing the number of genes (left) or exons (right) alternatively spliced after activation of the RG or the CNS promoters in comparison to cells transfected with scrambled sgRNAs. Exon usage of SQSTM1 after RG and CNS promoter activation reveals similar changes to transfections of scrambled sgRNAs (control) and additional differences between each other; comparison between ( b ) CNS and RG promoter activation, ( c ) RG promoter activation and control and ( d ) CNS promoter activation and control; different exon usage between pairwise comparisons is indicated by purple boxes representing the affected exon bins; significant differences ( p < 0.0001) are highlighted by stars; * and **, regions different between RG or CNS vs. scrambled; ***, region, different between CNS vs. RG or scrambled. The black lines refer to differences in any comparison.

Journal: International Journal of Molecular Sciences

Article Title: Selective Activation of CNS and Reference PPARGC1A Promoters Is Associated with Distinct Gene Programs Relevant for Neurodegenerative Diseases

doi: 10.3390/ijms22073296

Figure Lengend Snippet: CNS-specific and reference PGC-1α proteins affect exon usage via distinct and similar mechanisms. ( a ) Venn diagram showing the number of genes (left) or exons (right) alternatively spliced after activation of the RG or the CNS promoters in comparison to cells transfected with scrambled sgRNAs. Exon usage of SQSTM1 after RG and CNS promoter activation reveals similar changes to transfections of scrambled sgRNAs (control) and additional differences between each other; comparison between ( b ) CNS and RG promoter activation, ( c ) RG promoter activation and control and ( d ) CNS promoter activation and control; different exon usage between pairwise comparisons is indicated by purple boxes representing the affected exon bins; significant differences ( p < 0.0001) are highlighted by stars; * and **, regions different between RG or CNS vs. scrambled; ***, region, different between CNS vs. RG or scrambled. The black lines refer to differences in any comparison.

Article Snippet: For the stable integration of dCas9-VPR into the genome of cell lines, pLenti-EF1a-dCas9-SAM plasmids (ABM) along with the trans-complementation plasmids pMD2.G expressing VSV-G envelope and phCMV-8.91 expressing GAG/POL were transfected into HEK293T cells using jetPEI or Xfect transfection reagents (Polyplus Transfection T or Clontech, Mountain View, CA, USA) in serum and antibiotic free medium.

Techniques: Activation Assay, Comparison, Transfection